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在异源系统中作为谷胱甘肽S-转移酶融合蛋白的活性叙利亚金仓鼠朊病毒蛋白PrPc的过表达。

Overexpression of active Syrian golden hamster prion protein PrPc as a glutathione S-transferase fusion in heterologous systems.

作者信息

Weiss S, Famulok M, Edenhofer F, Wang Y H, Jones I M, Groschup M, Winnacker E L

机构信息

Laboratorium für Molekulare Biologie-Genzentrum-Institut für Biochemie der LMU München, Germany.

出版信息

J Virol. 1995 Aug;69(8):4776-83. doi: 10.1128/JVI.69.8.4776-4783.1995.

Abstract

This article describes a procedure which permits for the first time the isolation of the prion protein PrPc from the Syrian golden hamster in heterologous systems. Using a glutathione S-transferase (GST) fusion approach, milligram amounts of stable, soluble, and homogeneous GST::PrPc protein were obtained in Escherichia coli and with baculovirus-infected insect cells. Authentic PrPc was released from the immobilized fusion protein by direct cleavage with thrombin. GST::PrPc expressed in these two expression systems and also authentic PrPc released by thrombin cleavage were recognized by a polyclonal antibody directed against amino acid 95 to 110 of the golden hamster PrPc protein. GST::PrPc was not detected by a monoclonal antibody recognizing the region encompassing amino acids 138 to 152 of the human prion protein. The fusion protein was sensitive to proteinase K digestion, demonstrating that the cellular rather than the proteinase K-resistant scrapie isoform was produced.

摘要

本文描述了一种首次允许在异源系统中从叙利亚金仓鼠分离朊病毒蛋白PrPc的方法。采用谷胱甘肽S-转移酶(GST)融合方法,在大肠杆菌和杆状病毒感染的昆虫细胞中获得了毫克量的稳定、可溶且均一的GST::PrPc蛋白。通过凝血酶直接切割从固定化融合蛋白中释放出天然PrPc。在这两种表达系统中表达的GST::PrPc以及通过凝血酶切割释放的天然PrPc都被针对金仓鼠PrPc蛋白氨基酸95至110的多克隆抗体识别。识别人类朊病毒蛋白氨基酸138至152区域的单克隆抗体未检测到GST::PrPc。融合蛋白对蛋白酶K消化敏感,表明产生的是细胞型而非蛋白酶K抗性的瘙痒病异构体。

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